1

STERILITY TESTING OF
PHARMACEUTICALS
Made by: Netal Patel (09)
Pharm D. 3rd year
Parul Institute of Pharmacy
INTRODUCTION 2

• Sterilisation:
Is the process of making something free from bacteria or other
living microorganisms.

• Sterility Testing:
Are done to detect if viable forms of micro-organisms are
present or not on or in the pharmaceutical preparations.
INTRODUCTION 3

Which products undergo sterility tests?

• The test is applied to substances or preparations which, according to the
Pharmacopoeia, are required to be sterile. For example
✦ Injections
✦ Implants
✦ Syringes
✦ Bandages
✦ Dressings
✦ Surgical Instruments
✦ Needles
✦ Injectables
✦ Bulk Solids
✦ Ophthalmic Products..etc
INTRODUCTION 4

What precautions should be taken while performing sterility tests?

• The tests for sterility are carried out in aseptic regions to avoid accidental
contamination by microorganisms.
• The working conditions in which the tests are performed are monitored
regularly by appropriate sampling of the working area and by carrying out
appropriate controls.
PRINCIPLE 5

• If microorganisms are placed in a media that provides nutrients and water

and kept at a favourable temperature the organism will grow and their
growth can be indicated by turbidity in originally clear medium.
• The sterility tests provide optimum conditions for the growth and
multiplication of organisms, spores, etc that might be a contaminant.
• It is not possible to claim that a batch of products is sterile unless the entire
content of each batch has been tested.
• But these conditions are not possible because the article or the preparation
under test is either made unstable (like a syringe) or is destroyed (like an
injectable solution).
• Thus only a part of the batch can be sampled for testing.
STEPS INVOLVED IN STERILITY TESTING 6

1. Selection of the sample size.

2. Selection of the quantity of the product.

3. Method of testing.

4. Observation and Results.

1. SELECTION OF SAMPLE SIZE 7

Minimum quantity to be used for each

Quantity per Container medium unless otherwise justified and
authorised
Parenteral preparations:
• Not more than 100 containers • 10 per cent or 4 containers whichever is greater
• More than 100 but not more than 500 • 10 containers
containers
• More than 500 containers • 2 per cent or 20 containers (10 containers for large-
volume parenterals) whichever is less
Ophthalmic and other non-injectable:
• Not more than 200 containers • 5 per cent or 2 containers whichever is greater
• More than 200 containers • 10 containers
• If the product is presented in the form of single-
dose containers, apply the scheme shown
above for preparations for parenteral use

Bulk solid products:

• Up to 4 containers • Each container
• More than 4 containers but not more than 50 • 20 per cent or 4 containers whichever is greater
containers
• More than 50 containers • 2 per cent or 10 containers whichever is greater
2. SELECTION OF QUANTITY OF THE PRODUCT 8

Minimum quantity to be used for each medium

Quantity per Container
unless otherwise justified and authorised

Liquids:
• Less than 1ml • Whole contents of each container
• 1-40ml • Half contents of each container but not less than 1ml
• Greater than 40ml and not greater • 20ml
than 100ml
• Greater than 100ml • 10 per cent of the contents of the container but not less than
20ml
Antibiotics • 1ml
Insoluble preparations, creams and
Use the contents of each container to provide not less than
ointments to be suspended or
200mg
emulsified

Solids:
• Less than 50mg • The whole contents of each container
• 50mg or more but less than 300mg • Half the contents of each container but not less than 50mg
• 300mg-5g • 150mg
• Greater than 5g • 500mg
3. TEST METHODS 9

• Method A: Membrane Filtration method

• Method B: Direct Inoculation method
MEMBRANE FILTRATION METHOD 10

• Membrane has a nominal pore size not greater than 0.45 micron and diameter
of approximately 50mm.
• This method basically involves filtration of sample through membrane filters.
• The filtration is assisted under Vacuum after filtration completion the
membrane is cut into 2 halves and one halve is placed in two test tubes
containing FTM, SCDM medium.
• Incubate the media for not less than 14 days.
• Used for:
‣An oil or oily preparation.
‣Ointments that can be put into solutions.
‣Soluble powder.
‣Liquid products where volume in a container is 100ml or more.
‣Non bacteriostatic solid not readily soluble in culture media.
CULTURE MEDIUM 11

• Properties:
Must initiate and maintain vigorous growth of small numbers of aerobic or
anaerobic bacteria including spores.
Thus, must provide sufficient moisture, adequate pH, nutrients, suitable
Redox potential.
• Classification:
1. For detection of AEROBES:
Peptone Broth
Glucose Peptone Broth
2. For detection of ANAEROBES:
Cooked Meat Medium
Semi Fluid Meat Medium
Liver Broth
CULTURE MEDIUM 12

3. For both AEROBES and ANAEROBES:

Fluid Thioglycolate Media
Thioglycolate Broth Media
Corn Steep Liquor-Sodium Thioglycolate Media
Semi-FLuid Hydrosulphite Media
4. For detect of AEROBIC and LOWER FUNGI:
Soybean Caesin Digest Media
Sabourould’s Media
THIOGLYCOLATE MEDIUM 13

L-Cystine 0.5 g
Agar 0.75 g
Sodium chloride 2.5 g
Glucose monohydrate/anhydrous 5.5/5.0 g
Yeast extract (water-soluble) 5.0 g
Pancreatic digest of casein 15.0 g
Sodium thioglycollate or 0.5 g
Thioglycollic acid 0.3 ml
Resazurin sodium solution (1 g/l of resazurin sodium), freshly p 1.0 ml
Water R Upto 1000 ml

Sterilise in autoclave at 121 C for 20 mins

pH after sterilization 6.9 to 7.3.
ALTERNATIVE THIOGLYCOLATE MEDIUM 14

• Contains no agar and Indicator.

• Used with:
Turbid suspensions and viscid products (creams).
For devices having tubes with small Lumina.
SOYBEAN CAESIN DIGEST MEDIUM 15

Pancreatic digest of casein 17.0 g

Papaic digest of soya-bean meal 3.0 g
Sodium chloride 5.0 g
Dipotassium hydrogen phosphate 2.5 g
Glucose monohydrate/anhydrous 2.5/2.3 g
Water R Upto 1000 ml

pH after sterilization 7.1 to 7.5.

DIRECT INOCULATION METHOD 16

• It involves a direct inoculation of required volume of a sample in two test

tubes containing a culture medium that is FTM, SCDM.
• Volume of the preparation under examination is not more than 10% of the
volume of the medium.
• Incubate the inoculated media for not less than 14 days.
4. INTERPRETATION OF RESULTS 17

After incubation and during the incubation period

If growth is not observed If growth is observed

Passes the sterility test (preparation sterile) Containers are reserved and re-test is performed as
in the original test

If growth is not observed (sample passed) If growth is observed

If they are not readily distinguishable from those If they are readily distinguishable from those
growing in containers reserved in the first test growing in containers reserved in the first test

Preparation fails the test Second re-test is performed using twice the no.
of samples

If growth is not observed If growth is observed

Preparation passes the test Preparation fails the test

REFERENCES 18

• https://en.wikipedia.org/wiki/Sterilization_(microbiology)
• https://www.who.int/medicines/publications/pharmacopoeia/
TestForSterility-RevGenMethod_QAS11-413FINALMarch2012.pdf
• https://gibraltarlabsinc.com/services/microbiology/sterility-testing/
• https://www.eurofins.com.au/biopharma-services/testing-solutions/sterile-
products-testing/sterility-test/
• https://www.slideshare.net/parth241989/sterility-testing-112070804014
• Indian Pharmacopoeia,2010, Vol-I,p:56-63,36-37,28-33,196-198
• Lachman. L, Liberman HA, Kaniz JL, the theory and practice of industrial
pharmacy, Third Edition, Indian Edition p:635-638
• Mehta RM, Pharmaceutics-1,p:305, 311-315.